JP3659649B2 - Analytical devices and methods - Google Patents

Description

The present invention relates to analytical devices, and in particular, to an integrated one-step amplification analysis system that is particularly suitable for sensitive rapid test diagnostic devices. The present invention also relates to an analysis method, and relates to a kit used in an analysis device.
A one-step rapid test system can be used in medical tests such as in tests for pregnancy, sexually transmitted diseases, food tests, bacterial infections, antigen detection, livestock disease tests, environmental control, toxicity, biological drugs, etc. It is increasingly being used in a wide range of applications in immunoassays. However, in many other cases, the signal from the current rapid test is, for example, when detecting HIV antibodies in saliva or blood, or other in the urine or feces that show signs of a particular disease. Enough to produce qualitative or quantitative results, especially if the concentration of the substance to be detected is already extremely low in the sample, such as when detecting viral infections or small levels of bacteria Does not have high sensitivity.
One-step analysis preferably uses a simple, inexpensive, disposable device that requires little or no skill in operation. Application of the sample to the device is done in a single step. In this case, it is preferable that no cleaning or fluid change after use is required. The analysis result is given as a visible signal that can be easily read, and no special operation is required for reading.
Such rapid test devices typically include particles such as colored latex, carbon, or gold, and it is these particles that generate the final signal. A well known example of such a device is a pregnancy test kit that tests the level of the hormone βHCG in the urine. In such a device, gold or latex linked to an antibody against βHCG provides a source of visible signal.
Known examples of this type of device are disclosed in European Patent Specification No. 176799 and European Patent Specification No. 291194.
In order to directly generate a visible signal, it is important that the particles forming the signal source have a predetermined size. In the case of gold particles, the size of the gold particles should be greater than 10 nm and preferably greater than 40 nm in order to ensure the production of a clear visible signal. However, rapid one-step tests that limit the effectiveness of the particles are limited in sensitivity.
Rapid diagnostic tests are desired to be more sensitive to detect very small amounts of analyte. Although the concentration of analyte in saliva is typically 100 times less than the concentration of analyte in blood, non-invasive sampling is often preferred.
The present invention provides a very sensitive rapid detection device.
In the present invention, it is an analysis device for detecting the presence of an analyte in a sample and generating a visible signal at the detection site on the support that informs the presence or absence of the analyte. Generated or enhanced by a signal enhancement reaction between the labeled first binding agent and the label developing means, wherein the first binding agent and the label developing means are transported to the detection site by a single analysis step by application of the sample. In this case, the first binding agent and the label developing means are transported in an order such that the first binding agent arrives at the detection site before the label developing means. An analysis device characterized by the above is provided.
Among other things, the present invention
(A) a porous member;
(B) It binds specifically to the analyte and is movable through the porous member based on the influence of the liquid into the detection zone in a single step by only applying the sample, and is not visible. A first binding agent with a possible label;
(C) either specifically binds to the analyte complementary to the binding of the first binding agent, or is competitive with the analyte for binding to the first binding agent, and is detected A second binding agent immobilized within the site;
(D) a label developing means capable of moving into the detection site after the first binding agent under the influence of the liquid and making the invisible label visible.
An analysis device is provided.
In the above, the term “not visible” means that the label is usually not visible or only slightly visible to the naked eye, even when the concentration is high in the reaction zone or detection site during analysis. Yes. Examples of such labels are enzyme labels or particulate labels. They are not collected in a sufficiently large quantity to give a good visible signal, or are particularly small in size, for example less than 10 nm, suitably less than 5 nm, preferably 1-2 nm.
The label developing means includes a drug capable of developing the label so that the invisible label can be visually recognized. The nature of the developing means depends on the nature of the invisible label being used.
For example, when the invisible label is an enzyme label, the label developing means can include diaminobenzidine or another known enzyme developer.
In the case where the label includes a fine-grained label, the developing unit can deposit a material on the particles in order to make the particles visible. Suitable particulate labels include metal labels. The metal label is, for example, a gold, silver, selenium, or platinum label, or a particulate latex label, which can be enhanced if it is coated with an enhanceable material such as an enzyme or a metal coating. . Preferably, the particulate label comprises a particulate metal label, and most preferably the particulate label comprises a particulate gold label.
When a finely divided metal label is used, a suitable developing means comprises a silver agent such as silver lactate and a suitable developer such as hydroquinone. This is disclosed, for example, in Holgate et al., J. Hisotchem. Cytochem. 31, 938-944. The silver drug is suitably maintained in a dry form and in the appropriate zone of the porous member. The silver drug will remain in place until taken by the liquid passing through the zone towards the detection site.
Silver enhancement agents are commercially available from, for example, British Biocell International Ltd., Golden Gate, Ty Glas Avenue, Cardiff, UK.
Using a fine gold label in combination with a silver enhancement system to create an analytical test device according to the present invention increases signal strength by a factor of 100-1000, for a much wider range of applications than previously possible Can be applied. The speed of signal propagation will depend on the composition of the silver solution, the size of the gold particles, and the geometry of the device. The particle size can be, for example, in the range of 1-100 nm, and the particles are preferably small particles of less than 5 nm. The advantage of using small particles is that for a given sample, a much larger number of particles can collect in the detection zone for subsequent enhancement. This is due to the reduced spatial requirements. This results in a significantly increased signal compared to large particles that are not enhanced.
For such an analysis to be formulated as a one-step process, a sample that may contain an analyte and is labeled with a first binding agent is prior to the label developing means, It is necessary to ensure that the detection site is reached. Such a configuration can take many physical forms, and one such configuration is, for example, a liquid circuit as described in British Patent Application No. 2231150A. In a one-step analysis, it has not been disclosed to date to use a liquid circuit in supplying the label developing means for the preform signal.
Using this technique, channels of different lengths and / or widths are formed and liquid movement occurs through different zones formed by a series of substantially impermeable barriers. One particular form of liquid circuit is a printed liquid circuit, which consists of a filter paper or membrane printed on top with a wax pattern that forms a substantially non-permeable barrier. Or it has multiple layers. Agents required for analysis can be dried on the device at the appropriate location. The channel length and configuration can be used to control the arrival time of the liquid in various parts of the circuit, particularly in this case at the detection site. The channel width is used to control the liquid pressure.
A zone is provided so that the liquid sample that may contain the analyte and the first binding agent arrive at the detection site prior to the label developing means. When a liquid sample that may contain an analyte is applied separately from the first binding agent, the zone through which the liquid sample passes to ensure that an accurate signal is generated. The analyte must be configured so that it can arrive at the detection site prior to the first binding agent.
Thus, certain embodiments of the present invention provide:
(A) a porous member divided into a plurality of zones that are substantially impermeable to each other and intersect at a detection site;
(B) It binds specifically to the analyte and is located in one zone and is movable through the porous member based on the influence of the liquid into the detection site, and is not visible. A first binding agent with a possible label;
(C) either specifically binds to the analyte complementary to the binding of the first binding agent, or is competitive with the analyte for binding to the first binding agent, and is detected A second binding agent immobilized within the site;
(D) Label developing means that is arranged in a zone different from the one zone, can move into the detection site under the influence of the liquid, and can make an invisible label visible. When;
An analytical test device comprising:
Preferably, the first binding agent and the label developing means are each movable toward the detection site under the influence of the agent moving along the porous member. In addition, the liquid that may contain the analyte is directed to the detection site in combination with the first binding agent or along a further zone provided in the device for this purpose. Can be moved. Also, different liquids can be applied to each zone, or to each group of zones, and these can be applied individually into the sampling region or sampling well within each zone. Can do.
However, in a preferred embodiment, the device is configured such that at least the first binding agent and the label developing means move towards the detection site under the influence of the same liquid containing the sample under test. Has been. This results in a one-step rapid analysis system.
The zone or zone group is preferably such that the same sample can be applied simultaneously to the sampling areas of all zones or zone groups that form the starting point of the sample through the porous member to the detection site. In the device. For example, although one zone's non-permeable barrier configuration can form a longer liquid path than the other, the zones are substantially juxtaposed side by side.
Thereby, the analysis test device to be used can be a rapid analysis one-step system. This is because the sample can transport both the first binding agent and the label developing means towards the detection site.
However, other methods can be used to ensure sequential transport of the first binding agent and the label developing means toward the detection site. As such a method, there is a method of using a sustained-release composition. In this case, it is ensured that the release of the label developing means is slower than the release of the first labeled binding agent.
Such release agents include gelatin and other enzymes, polyethylene glycol (PEG), polyvinylpyrrolidine (PVP), and other polymers, surfactants, gum arabic, sucrose and other sugars, clays , Lipids, resins, salts, and other sustained release drugs such as those used in the pharmaceutical industry. Such sustained release drugs are typically applied at a concentration of 0.1-5%, preferably on the order of 1% w / v.
Another control method for releasing the drug from the membrane so that it can flow toward the detection zone is to change the water repellency of the membrane in the detection zone so that wetting of the zone by the sample can be controlled. is there. In such methods, for example, Triton X 705, high salt concentrations (eg 5% NaCl), certain fatty acids, or polyamino acids such as poly L tryphophan (Sigma), high Certain water repellent surfactants are used, such as all that have water repellent properties and can be impregnated into the membrane.
Alternatively, the movable labeled binding agent and the label developing means can be placed inside or behind a semi-permeable barrier such as gelatin, glycerol, polymer, or the like. Thus, the movable labeled binding agent and the label developing means are gradually released as the sample enters the barrier to dissolve the agent. The choice of barrier material thus determines the dissolution rate and determines the release of the drug upon movement towards the reaction zone.
In other embodiments, the movable labeled binding agent and / or label developing means is applied on a separate layer of porous material. In this case, the individual layer is in relation to the porous member that the liquid moving through the porous member first passes under the individual porous layer and gradually as the liquid flows. In contact with the first binding agent or label developing means that is absorbed into the liquid and eventually applied to the liquid as it flows through the device. As the other porous layer, a film, paper, or a glass fiber pad can be appropriately used.
In still another embodiment, the labeled first binding agent and the label developing means are arranged on the porous member so that the labeled first binding agent rides on the laminar flow of the liquid sample directly toward the detection zone. It is arranged so that it can move and the label developing means does not come into contact with the detection zone. However, if a suitable barrier is placed in the path of the developing means, the developing means can be deflected towards the detection zone. In this case, the deflection process inevitably delays the liquid travel. The barrier can essentially be placed in the path of the liquid carrying the label developing means. However, it is preferable that the label developing unit itself contributes to the construction of the barrier. As a result, only a slight time difference occurs between the arrival of the labeled first binding agent and the arrival of the label developing means.
This embodiment is most preferred when the label is a finely divided metal such as gold, and the developing means is of a type in which a material film is formed on the surface of the metal particle such as a silver drug. For example, small metal particles form a barrier on the porous member in the path of the label developing means so that when the particles are enlarged, they guide the label developing means toward a detection zone (described later). And it is fixedly arranged. In use, the label developing means first encounters these particles to form a film on the particles. As film formation proceeds, the expanded particles form a barrier against a continuous laminar flow of liquid containing the label developing means. Therefore, the label developing means is deflected.
This principle can be used in a wide range of analyses, for example, where liquid deflection is desired during an analysis with sequential reactions or reaction steps. It is not necessary for the label developing means to be required to enhance the generated signal. In this case, the situation is clearly simplified. If two functions are required, the two functions are incorporated into a single label developing means.
Analytical devices using this principle form another aspect of the present invention.
The device of the present invention can be used for “sandwich” or “competition” analysis methods. In sandwich analysis, the second binding agent binds to the analyte in a manner that is complementary to the first binding agent. In this case, the first binding agent moves into the detection zone based on the influence of the liquid sample that may contain the analyte. Anything bound to the analyte is collected in a detection site where the label developing means has already arrived. Thereby, a visible signal is formed.
In competitive analysis, the second binding agent competes with the analyte upon binding to the first binding agent. Even in this case, the first binding agent moves into the detection zone based on the influence of the liquid sample under test. In this case, however, everything bound to the analyte is not retained in the detection site. Only unbound first binding agent is collected at the detection site and forms a visible signal. In this case, the larger the signal, the less analyte is present in the sample.
In this type of analysis, other binding agents that specifically bind to the first binding agent or other binding agents that specifically bind to the analyte in a manner that is complementary to the first binding agent. Binding agents can also be used. Such other drugs are fixed to a catch site arranged at a position beyond the detection site and along the sample path. Such other agents will collect the analyte / first binding agent complex or conjugate bound at the catch site. When the label developing means arrives, a visible signal is generated at the catch site. In this way, the signal generated by the bound first binding agent compared to the unbound first binding agent provides a more qualitative assessment of the analyte present in the sample under test.
Filter means can be provided in the device of the present invention as needed or desired. For example, it can be provided in some zones of the device that have a non-permeable barrier. Or it can provide in the front side of the chemical | medical agent applied to the film | membrane surface with respect to the distribution direction of a sample solution. This can remove unwanted elements from the sample within these zones or regions. Such filter means may comprise a physical filter or an immunological or biochemical agent that binds to undesirable elements. For example, if serological analysis is being performed on a serum sample, the serum is used, for example, as a carrier liquid for the first binding agent of the label developing means, or even as a washing liquid described below. There is a wide range of serum antibodies. In such cases, they can be removed from the serum by providing an immunological barrier in the relevant zone. An immunological barrier is fixed on the porous member, for example, to ensure that serum can flow through the barrier before reaching the detection site, eg, an anti-human IgG antibody An anti-IgG antibody such as can be provided.
The use of such filter means during analysis forms another aspect of the present invention.
By using techniques such as liquid circuit technology, additional steps can be incorporated into the analysis. For example, one or more zones can be provided and arranged to transport the cleaning liquid toward the detection site. For example, it is desirable that the cleaning liquid be transported after the first binding agent passes and before the label developing means arrives. This has the effect of removing from the detection site all labeled first binding agents that are not bound to the detection site before the signal is formed. This cleaning liquid can contain the sample itself. Here, the sample is additionally filtered as it passes through the associated zone to remove contaminants and excess drug.
The additional washing step is particularly suitable in the case of serum analysis, for example in the case of serum analysis of serum samples. Thereby, excess serum and non-specific antibodies can be removed from the detection site.
Similarly, label development leading to signal generation, if appropriate, by providing other zones for transporting the liquid, which is preferably the sample itself, again to the detection site as a final step. Can be terminated.
The device of the present invention can be configured such that a series of reactions are performed sequentially and with a time lag. In this case, the time difference depends on the length of the liquid channel formed in each liquid impermeable zone of the porous member, for example in the case of a liquid circuit. Alternatively, it depends on the nature of the sustained release or the nature of the barrier to various drugs.
In a preferred embodiment, a wick or wick zone into which the liquid or excess drug is poured before or after the liquid or excess drug participates in the reaction can be provided. This improves liquid flow through the device.
The choice of first binding agent and second binding agent in each case depends on the nature of the analyte under test. If the analyte comprises an antigenic protein or polypeptide such as a hormone-like βHCG, the first and second binding agents are, as in the past, in sandwich analysis or competitive analysis techniques, as these proteins Specific antibodies or antibody-binding fragments can be provided. Alternatively, the device of the invention can be used for serological analysis where the analyte itself is equipped with a specific antibody, such as an HIV antibody. In such a case, preferably, the second binding agent comprises an antigen to which the target antibody specifically binds, and the first binding agent binds to the analyte antibody. It has. In such cases, the analyte antibody is suitably immobilized at the detection site prior to the introduction of the labeled anti-antibody. Labeled anti-antibodies are applied to arrive at the detection zone with some time delay, for example by being administered to other zones of the liquid circuit.
Additionally, the analyte can be a nucleic acid such as RNA or DNA. In this case, the first and second binding agents can comprise nucleic acid binding components such as labeled nucleic acid probes that are hybridized to the nucleic acid under test.
Suitable porous members for use in the device include porous membranes and paper, as is well known in the art. Among suitable porous members are nitrocellulose membranes.
The device can be equipped with a simple dipstick. Depending on the shape of the device, it is slightly wider than a conventional dipstick that is attached to a plastic backing plate without a protector against the surface. Alternatively, the device can be enclosed in a container such as a plastic housing. An opening for applying a sample is provided in the housing. Alternatively, it can be in the form of a laminated card. In this case, the end of the sample is exposed by cutting or tearing the laminate immediately before use and then immersed in the sample. As still another form, a flat card can be used. All chemicals, barriers, and circuits are mounted on the flat card. The card is coated with a non-permeable membrane, such as a sprayed plastic membrane.
The invention will now be illustrated in detail with reference to the accompanying schematic drawings.
FIG. 1 is a diagram schematically showing a configuration of an analytical test device before use.
FIG. 2 schematically shows the device of FIG. 1 at the end of the analysis.
FIG. 3 is a diagram schematically showing the configuration of an analytical test device using competitive analysis.
FIG. 4 schematically shows an analytical test device applied in particular to serum analysis and including a washing step.
FIG. 5 schematically illustrates another embodiment of a test device for use in serum analysis.
FIG. 6 schematically illustrates a test device for use in connection with serum analysis utilizing a serum sample as a carrier medium.
FIG. 7 is a diagram schematically showing an analytical test device for performing one-step sandwich analysis with a signal enhancement function and performing sequential release and controlled diffusion of drugs.
FIG. 8 is a diagram schematically showing an analytical test device similar to FIG. 7 in which a diffusion zone is provided in a funnel shape.
FIG. 9 schematically illustrates an analytical test device in which sequential delivery of drugs to the detection zone is obtained using an enhanced reaction to automatically change fluid flow during use.
10A and 10B are a front view and a side view, respectively, schematically showing an analytical test device that sequentially releases and linearly distributes drugs from the membrane surface for sequential signal enhancement in sandwich analysis. .
FIGS. 11A and 11B schematically show an analytical test device that sequentially releases drugs from the membrane surface and overlay pad surface for sequential signal enhancement in sandwich analysis, in front and side views, respectively. is there.
FIG. 12 schematically illustrates an analytical test device with a drug deposited behind a slowly melting barrier for progressive release and distribution for sequential signal enhancement in sandwich analysis.
FIG. 13A shows an analytical test that sequentially releases drugs from superimposed or overlapped lower wicks on a membrane with immobilized target binding protein for sequential signal enhancement in sandwich analysis. FIG. 13 schematically shows the device, and FIG. 13B shows a side view thereof.
The test device (FIG. 1) includes a porous membrane 1. In the porous membrane 1, the reaction site 5 is divided into a first zone 3 and a second zone 4 by an impermeable barrier 2.
An antibody 6 for an analyte is provided in one end 7 of the first zone. The antibody 6 is linked to gold particles 8 having a size of 5 nm or less. A reaction antibody 9 that also links an analyte is fixed on the porous membrane 1 in the reaction site 5.
A dry silver reactant 10 such as milky silver and a developer such as hydroquinone are disposed at the end 7 of the second zone 4. Within the second zone 4 there is a series of impermeable barriers 11 forming a channel 12.
In use, the end 7 is immersed in a liquid sample that may contain the analyte. The sample passes through the porous membrane 1. The sample passing through the first zone 3 collects the labeled antibody 6 and carries the antibody 6 to the reaction site 5. If the analyte 13 (FIG. 2) is present in the sample, it will bind to the antibody 6. In the reaction site 5, the analyte-antibody complex is linked to the reaction antibody 9.
The sample passing through the second zone 4 collects the silver reactant 10 and then passes through the channel 12 as indicated by the arrow. Therefore, it takes a longer time to reach the reaction site 5. When the analyte is present, when the sample passing through the second zone 4 reaches the reaction site 5, the reaction site 5 has gold-labeled particles at a predetermined concentration. The silver reactant 10 reacts with these particles to develop a brown black visible signal 14.
In the alternative device shown in FIG. 3, a competitive analysis can be performed. This embodiment includes a porous card 1. On the porous card 1, three channels 15, 16, and 17 are formed. The first channel 15 has an antibody 18 labeled with gold, such as a mouse antibody. The second channel 16 has a milky silver / hydroquinone mixture 19. An antigen 20 that competes with an analyte for binding to the antibody 18 is immobilized at the detection site 21. An anti-antibody 22 such as an anti-mouse antibody is immobilized at the reaction site 23.
The channels 15, 16, and 17 are provided so that the liquid can move along the channel and sequentially reach the detection site 21 and further the reaction site 23. A wick zone 24 is provided to receive the liquid after it has passed through the reaction site 23.
In use, the lower end 25 of the card 1 is immersed in a liquid sample that may contain an analyte. As a result, the liquid sample enters the channels 15, 16, and 17. All analyte in the sample in the shortest channel 15 binds to the antibody 18 labeled with gold. Then, it moves along the channel 15 and encounters the antigen 20 fixed at the detection site 21. Labeled antibody 18, already bound by the analyte, will pass through this region. In contrast, unbound labeled antibody 18 remains within this region.
Bound labeled antibody 18 that has passed through detection site 21 encounters anti-antibody 22 and thus remains at reaction site 23.
The sample passing through the second longest channel 16 carries the silver / hydroquinone reactant 19 to both the detection site 21 and the reaction site 23. At these sites, the silver / hydroquinone reactant 19 encounters the antibody 18 labeled with gold that remains at these sites. Gold labels drive the generation of brown-black visible signals. In this case, the intensity of the brown-black visible signal depends on the amount of antibody 18 present at these sites.
Finally, sample transport in the third channel 17 occurs at the detection site 21 and the reaction site 23, washing the silver enhanced gold binding complex at these sites. All excess liquid is directed to the wick area.
FIG. 4 shows still another embodiment of the analysis device of the present invention. This embodiment is particularly applicable to serum immunoassays for the detection of serum antibodies. This embodiment includes a porous support 26. On this porous support 26, three channels 27, 28 and 29, which are gradually increased in length, are formed. Each channel is provided with a liquid receiving opening 30, 31, 32 in the end region of each channel.
In the detection zone 34, an antigen 33 to which a serum antibody or an analyte is bound is fixed. Located in the second channel 28 is an anti-antibody 35 labeled with gold. In the third channel 29, milky silver / hydroquinone color former 29 is dried. In use, a serum sample is introduced into the opening 30 of the first channel 27. Then, the cleaning liquid is disposed in the other openings 31 and 32. The sample moves along the first channel 27 and encounters an antigen 33 to which a particular antibody in the sample will be linked. Other than the specific antibody in the sample proceeds to the wick region 37.
In parallel, the wash fluid from the opening 31 of the second channel 28 carries the antibody 35 labeled with gold to the detection site 34. At the detection site 34, the antibody 35 labeled with gold encounters and binds to all serum antibodies immobilized thereon. The silver / hydroquinone 36 is transported by the cleaning liquid from the opening 32 in the third channel 29 and arrives late. The silver / hydroquinone 36 then reacts with all the bound gold complexes to give a visible signal that indicates the presence of serum antibodies in the sample.
FIG. 5 shows a variant of the analysis device of FIG. This embodiment comprises intermediate and intermediate wash steps between analytical binding reactions. This has been obtained by introducing additional channels 40, 41, 42. All the channels are arranged so as to be able to receive the washing liquid arranged in the receiving area 39. Channels 40, 41, 42 are configured to carry cleaning liquid to detection site 34. This allows (a) the antigen / serum antibody complex formed at the detection site to be washed before the gold-labeled antibody 35 arrives, and (b) before the silver / hydroquinone color former arrives. In addition, the antigen / serum antibody complex / gold labeled antibody can be washed, and (c) the silver enhancement complex can be washed at the detection site 34 to terminate the enhancement.
This embodiment can be modified as shown in FIG. 6, which can provide a washing step for the serum sample if necessary. In this case, it is ensured that all sera except those passing through the first channel 27 come into contact with the immobilized anti-human IgG in order to remove serum antibodies that can cause the remaining sera to act as washings. It is necessary. Immobilized anti-human IgG43 is suitably provided in the form of a lateral barrier that extends across each associated channel. This eliminates the need to provide a separate reservoir for the cleaning liquid.
In an alternative embodiment, the device can comprise a membrane with an appropriate agent introduced. Such drugs are arranged such that the drugs move sequentially towards the detection zone under the influence of the applied sample. One such embodiment is shown in FIG. A solid phase carrier 45 such as paper, nitrocellulose, glass fiber, or other porous material such as the above mentioned membranes ensures that some remain movable and others are not. And is properly coated with the drug. The device can be any suitable shape. For example, it can be coated with an impermeable barrier, as shown by the dashed line 46 in FIG. 7, to narrow the flow of drug towards the detection zone.
The sample can be applied to the lower end 47, or alternatively can be applied to a number of openings in the lower end of the carrier. In this case, the sample is moved by capillary action towards a mobile labeled binder 48 such as a gold labeled antibody and a labeling means such as a silver enhancer or mobile enhancer 49. Yes. The sample moves along the carrier 45. In doing so, it moves beyond the mobile labeled binding agent 48 and mobile enhancement agent 49 and in the detection zone it moves directly towards a fixed binding agent 50 such as a reactive antibody. In order to properly position the members, the mobile agents 48, 49 can deposit agents with different release characteristics on the carrier to allow for time-released drug release from the carrier. Appropriate selection of drug release can control the extent and rate of release of labeled drug 48 and augmented drug 49, and can control the environment in which they are temporarily immobilized and then react. it can.
In this way, the medicine sequentially moves in the direction of the arrow toward the detection zone. And preferably, it moves through the detection zone to the upper zone 51 by being pulled by capillary action. In order to assist in proper interaction and uniform contact of the binding agent 50 to the mobile agents 48, 49, a diffusion means 52 can be provided, which is arranged on the sample path just before the detection zone. Can be arranged. This diffusing means 52 can be, for example, for proteins (eg bovine serum albumin or BSA), polymers (eg polyvinyl alcohol (PVA), PEG, PVP, etc.), salts, or even flow through the detection zone Alternatively, it can take the form of fixed materials such as glycerol, gum arabic, other suitable materials such as lipids deposited on the membrane such that drug dispersion can be caused. The membrane can also incorporate a woven pattern of permeable or non-permeable material to cause such mixing or diffusion in the diffusion zone. Such non-permeable materials include waxes. This wax is deposited on the film using a high resolution high temperature wax printer driven based on a graphic computer program that will produce the desired pattern. A suitable high temperature wax printer is the Phaser 340 available from Tetronix Europe, UK. A suitable graphic design package is Autosketch available from Autodesk Inc, USA. Alternatively, diffusion can be obtained by placing a separating material such as a glass fiber pad provided on the membrane in the diffusion zone.
Analyte present in the sample first reacts with the first labeled agent 48 and then advances through the detection zone. Due to the interaction between the analyte and the binding agent 50, a sandwich can be formed. Because the label of the first binding agent 48 is invisible (eg, an enzyme or a small gold or unenhanced label), no direct signal is detected. As the sample continues to move beyond the detection zone, this post-sandwich cleaning effect is created. Subsequent release of the enhancement agent 49 allows the enhancement agent 49 to move further through the detection zone towards the detection zone. This can cause the desired signal enhancement to provide an indirect signal. After this enhancement, further sample movement can clean the membrane and form a clear signal on the background of the reaction zone.
Alternatively, the device can take the form of a film consisting of a single narrow strip as shown in FIG. In this case, the movable drugs 48, 49 are juxtaposed in close proximity at the bottom of the strip. By using an appropriate sustained release agent, each agent can be moved sequentially toward the binding agent 50 in the detection zone. The drug is diffused before reaching the detection zone by disposing the diffusing means 52 immediately before the detection zone. In this case, the laminar flow ensures that the drugs do not mix before they sequentially reach the diffusion means.
Surprisingly, the silver-enhancing agent caused the deposition of metallic silver on the gold-labeled binding protein in the detection zone, thereby causing the silver to flow further through the detection zone. It was found that a semi-permeable barrier was formed. This has the effect of changing the flow path of the drug through the detection zone, and as a result, the final reaction product substantially changes the device shape. This is the entire detection zone. Throughout the detection zone, silver ions diffuse uniformly and the silver ions can even enhance the gold particles in the detection zone. In this way, a thin flow of drug through the detection zone automatically diffuses throughout the detection zone.
In further attempts, the silver enhancement agent caused the formation of metallic silver that substantially altered the flow of liquid through the membrane by permanently depositing gold particles at appropriate locations on the membrane. In this manner, the drug can be sequentially transported to the detection zone without using an impermeable barrier and without using a sustained-release drug.
One such embodiment is shown in FIG. In this embodiment, the labeled drug 48 is positioned on the carrier 45 such that the labeled drug 48 can be advanced directly toward the binding agent 50 in the detection zone under laminar flow. ing. The enhancement agent 49 is arranged so that the enhancement agent 49 can bypass the detection zone when the enhancement agent 49 is advanced along the laminar flow. However, when the sample continues to flow along the carrier, the gold particle 53 has a barrier in the flow path of the enhancing drug 49 where the flow in the detection zone has substantially converged as indicated by the arrow. As formed, it is placed in the path of the enhancement agent 49 on the carrier.
Alternatively, the device can have a simple dipstick shape as shown in FIG. In this case, all drugs are deposited in the lateral direction in different zones. Controlled release of these drugs is then effected by application of appropriate release drugs in each zone. Thus, the sample is applied to the lower end 47 of the strip and pulled by capillary action to flow through each zone and then to the upper part 51. The sample continues to flow through the enhancement agent 49 to the labeled binding protein 48 without immediate release. At the labeled binding protein 48, an interaction occurs between the analyte in the sample and the labeled binding protein 48. At the same time, the labeled binding protein is released. The labeled binding protein then moves toward the reaction binding protein 50. When a specific analyte is present in the sample, further interaction occurs at that location to form a sandwich as described above. Excess sample solution passes through the reaction zone to the upper region 51 of the strip 51. The upper region 51 of the strip 51 can have overlapping wicks or a larger surface area (not shown) to effectively pull the sample from the detection zone.
Subsequent release of the enhancement agent 49 occurs by continuous flow of the sample liquid. This release is controlled by the choice of sustained release drug as described above. The enhancement agent 49 is similarly pulled from the detection zone to form a visible signal.
Many drugs can be deposited in the lower part of the membrane in this way so that many subsequent reactions occur. Using a small gold special label after silver enhancement, or using an enzyme label after a color reactant, is a large diameter gold or a specific label in currently available prior art rapid test systems Results in a greater indirect signal strength compared to the direct signal provided by. In addition, in this method, washing can be performed between the various reactions in the reaction zone. This cleaning is performed by the sample itself. For simultaneous detection of two or more analytes from a sample, it is additionally possible to provide two or more reactive binding agents immobilized within the detection zone.
Alternatively, the movable labeled binding agent and / or enhancement means can be deposited on a separate layer such as a permeable membrane, paper, or glass fiber. In this case, the individual layer is in contact with the surface of the device film. Thereby, the sample solution first moves under this second layer towards the reaction zone and passes through the reaction zone after a controlled time lapse. Thus, the labeled binding agent or the labeled developing means is released. This embodiment is illustrated in FIG. In the figure, the enhancement agent 49 is disposed on a glass fiber pad 54 that is fixed on the surface of the carrier 45. The time interval between the release of the labeled binding agent or the label developing means can be controlled by selecting the material forming the second layer or by selecting the releasing agent within the second layer. The rate of drug migration through the device membrane can be pretreated with the membrane or second layer material using, for example, a suitable inhibitor, such as a surfactant, polymer, protein, saccharide, resin, alone or in combination. Is controlled.
Extending this principle, multiple layers of such membranes can be incorporated in one place. In this case, each layer comprises different reactants that are sequentially dissolved and transported to the device membrane. These multiple layers may or may not be separated by an uncoated membrane so that more precise sequential release onto the device membrane can be achieved. One advantage of such a layered configuration is that one or both of the labeled binding agent and the label developing means are not initially incorporated within the body of the device membrane. Accordingly, the sample solution can be freely distributed to the reaction zone.
Such devices can be used in sandwich analysis or as a liquid circuit configuration in competitive analysis, as described above. In the competitive analysis format, the second binding agent 50 competes with the sample analyte for binding to the first binding agent 48. During the test, the first binding agent 48 moves to the detection zone under the influence of the liquid sample. However, in this example, everything already bound to the sample analyte is not retained in the detection zone. Only unbound first labeled binding agent 48 will accumulate in the detection zone and form a visible signal. In this example, the larger the signal, the fewer analytes present in the sample, indicating that the sample is deficient. The immediately labeled binding agent 48 is not visible in the detection zone. However, the subsequent enhancement due to the sequential arrival of the enhancement agent 49 reduces the visible label to a greater strength compared to the prior art direct type labels currently in use.
The device according to the invention can also be used for the detection of specific antibodies (s) in serum, saliva or other biological fluids or sample solutions prepared from other sources. A particularly preferred embodiment in this case is shown in FIG. The form of the device is roughly the same as that shown in FIG. In this case, however, the immobilized reactive agent can be an antigen specific to the antibody to be detected. Labeled binding agent 48 is a suitable binding protein such as protein A or AG, or anti-human IgG, etc., labeled with small gold particles, or other particulate materials, or enzymes, etc. It can be. The enhancement agent 49 can again be a silver enhancement agent, an enzyme substrate, or a dye, as described above. By sequentially releasing these binding agents, a reaction with a time difference can be caused in the detection zone.
Samples containing specific and non-specific antibodies first migrate through the intact gap 55 and react directly with the immobilized antigen 50a in the detection zone. Then, by releasing the labeled drug 48, the labeled drug 48 can be reacted with the sample antigen fixed at this time in the detection zone. Controlled subsequent release of labeled binding agent 48 and enhancement agent 49 can be achieved with a release material similar to that described above or by depositing behind or within a semi-permeable barrier similar to that described above. , Has been brought. The sample passes through the detection zone, providing a cleaning effect prior to subsequent release of the enhancement agent 49 that provides a visible signal.
In order to reduce the adhesion of non-specific antibodies present in the sample to the labeled binding agent 48, the labeled binding agent 48 can be partially shielded by a band 56 made of anti-IgG. In this configuration, the sample passes through the anti-IgG band 56 to cause the release and distribution of the labeled binding agent 48 and subsequently causes the release and distribution of the enhancement agent 49. However, specific IgG and non-specific IgG are filtered from this part of the sample.
If the desired wick zone for sample application to both the bottom and top of the membrane is provided for full withdrawal of the sample by capillary action through the detection zone, the device is shown in FIG. Appropriate shapes can be used, and sample and drug can be focused through the diffusion means 52 and the detection or reaction zone.
Alternatively, the device can take the form shown in FIG. In this form, all of the drug is deposited across the strip in different zones. And the controlled release of these drugs is brought about by the application of the appropriate release material for each zone. Thus, the sample is applied to the lower end of the strip and pulled through the zones and into the upper part 51 by capillary action. In this case, the drug is positioned so that the sample can pass through the augmenting agent 49 and the labeled binding agent 48 without immediately releasing both the augmenting agent 49 and the labeled binding agent 48. The sample proceeds towards the detection zone. At this detection zone, the in-sample analyte is specifically bound to the reactive agent 50. Further sample solution flow causes subsequent release of the labeled binding agent 48. Then, the labeled binding agent 48 further flows through the reaction zone toward the reaction zone. Then, it binds to a specific antibody extracted from the sample and fixed in the reaction zone. Furthermore, the flow of the sample solution results in the subsequent release of the enhancement agent 49. The enhancement agent 49 then flows to the reaction zone and reinforces the label to generate a visible signal.
In a preferred embodiment, the device takes the form of a simple dipstick as shown in FIG. In this embodiment, the mobile agents 48, 49 are deposited in different zones on a lower pad or wick 57 comprising, for example, glass fibers. The movable drugs 48 and 49 are contained in a sustained release material such as gum arabic as described above. Sustained release materials appropriately control the release of different drugs. The sample is applied to the lower end 47 of the strip and pulled by capillary action and passes through each drug zone to the detection zone. The sample passes through the lower wick 57 and proceeds to the labeled binding agent 48 without releasing the enhancement agent 49 immediately. At the labeled binding agent 48, an interaction between the analyte in the sample and the labeled binding agent 48 occurs, and at the same time, the labeled binding agent 48 is released. The resulting solution then moves on the membrane 58 and moves toward the binding agent 50. If a particular analyte is present in the sample, then further interaction takes place and forms a sandwich as described above. Excess sample solution flows through the detection zone toward the upper region 51. The upper region 51 is provided with an overlap wick 59 or a larger surface area so that the sample can be drawn beyond the effective detection zone. When the sample solution subsequently flows, the enhancement drug 49 is released from the lower wick and flows out. Thereby, the enhancement agent 49 moves relative to the membrane and flows toward the detection zone. At the detection zone, the enhancement agent 49 causes label enhancement. Further sample flow causes washing of excess augmentation drug from the target zone.
Similarly, a simpler configuration using a sustained release agent as the labeled binding agent can be formed by using a visible label in any of the embodiments shown in FIGS. 7-13 above. . In this case, no subsequent enhancement is necessary to visualize the signal.
The analysis device of the present invention can be provided as a finished product. Alternatively, it can be provided in the form of a kit. The analytical device comprises a porous member comprising, for example, a suitable impermeable barrier and / or a mark or band or antibody representing the location to which the drug is to be applied. The appropriate drug may or may not be included as part of the kit.
The following examples are described for illustration only.
Example 1
A device substantially in the form of FIG. 10 was constructed as follows. Nitrocellulose membranes having a pore size of 8 μm and supported on a hard plastic backing plate were obtained from Advanced Micro Devices, New Delhi, India. The membrane strip was cut to 5 mm width and 80 mm length. For simple illustration of the invention, rabbit IgG (Sigma Chemicals Ltd, Poole, UK) was diluted to 1 mg / ml in deionized water. This is then used with a piezoelectric inkjet printer (Bioprinter, British Biocell International Ltd, Cardiff, UK) specially configured for protein printing for diagnostic devices, with a strength of 1 μl / cm and 4 cm from the bottom. However, it was applied in a striped manner on the strip. The protein stripe was dried at 37 ° C. for 15 minutes. The stripe was then blocked by immersion in a solution consisting of 0.1% Tween 20 and 1% polyvinylpyrrolidine (Sigma UK). The strip was dried at 37 ° C. for 30 minutes. Goat anti-rabbit IgG with 1 nm gold particles (British Biocell, UK) attached was diluted to an antibody concentration of 1 μg / ml in a solvent consisting of 0.1% Tween20 and 1% polyvinylpyrrolidine (Sigma UK). 5 μl was weighed and applied on a strip about 3 cm from the lower end. An optical microscope silver enhancement kit SELK15 (British Biocell International Ltd) with initiator and developer was obtained. The initiator and developer were individually diluted 1: 1 for an aqueous 1% solution of gum arabic (Sigma Chemical, UK). 2 μl for each drug was weighed onto the membrane strip. The initiator was placed 1 cm from the lower end, and the enhancer was placed 2 cm from the lower end. The strip was dried at 37 ° C. for 30 minutes. The strips were then placed in 100 μl microwells of phosphate buffered saline. Gold labeled goat anti-rabbit IgG was transferred to immobilized rabbit IgG and held for less than 1 minute. However, a clear signal was not obtained. In addition, when held for 2 minutes, the initiator and enhancer migrated over the strip and reacted with the gold labeled antibody, producing a strong black signal.
Example 2
A sandwich analysis device was made in the form of FIG. 10 to detect beta HCG in urine. Using a Bioprinter against a nitrocellulose membrane (AMD, India) with a pore size of 8 μm and supported on a plastic backing plate, 1 mg / ml of a single clone anti-alpha HCG (Sigma Chemicals Ltd, UK) The solution was stripped at a concentration of 1 μl / cm in water. The strip was dried at 37 ° C. for 15 minutes. The membrane strip was then blocked by immersion for 1 minute in a mixed solution consisting of 0.1% Tween 20 and 1% polyvinylpyrrolidine (Sigma Chemicals Ltd, UK). Then, it was dried at 37 ° C. for 30 minutes. Monoclonal anti-alpha HCG with 1 nm gold particles (British Biocell, UK) attached was diluted to an antibody concentration of 1 μg / ml in a solvent consisting of 0.1% Tween20 and 1% polyvinylpyrrolidine. 5 μl was weighed and applied on a strip about 3 cm from the lower end.
Both enhancer and initiator were applied to the strip and the strip was dried at 37 ° C. for 30 minutes. The strip was then placed in a microwell containing 100 μl urine from a 4 week pregnant woman. The sample caused migration of the gold complex from the strip toward the reaction zone and reacted with the beta HCG analyte in the sample. Within 3 minutes, the sample transferred the silver enhancing agent from the membrane strip to the reaction zone, producing a strong black line indicating the presence of the analyte. Further sample distribution washed the strip to wash all background stains.
Example 3
Another sandwich analysis device was made in the form of FIG. 10 to detect hepatitis B surface antigen in a standard sample. A nitrocellulose membrane (AMD, India) with a pore size of 8 μm and supported on a plastic backing plate, using Bioprinter, 1 mg / kg of monoclonal anti-hepatitis B surface antigen (Genzyme, UK) The ml solution was stripped at a concentration of 1 μl / cm in water. The strip was dried at 37 ° C. for 15 minutes. The membrane strip was then blocked by immersion for 1 minute in a mixed solution consisting of 0.1% Tween 20 and 1% polyvinylpyrrolidine (Sigma Chemicals Ltd, UK). Then, it was dried at 37 ° C. for 30 minutes. A second single-clonal anti-hepatitis B surface antigen with 1 nm gold particles (British Biocell, UK) attached to an antibody concentration of 1 μg / ml in a solvent consisting of 0.1% Tween20 and 1% polyvinylpyrrolidine. Diluted. 5 μl was weighed and applied on a strip about 3 cm from the lower end. Both enhancer and initiator were applied to the strip and the strip was dried at 37 ° C. for 30 minutes. The strips were then placed in microwells containing 100 μl PBS supplemented with a standard concentration of hepatitis B surface antigen (Genzyme, UK). The sample caused migration of the gold complex from the strip towards the reaction zone and reacted with the hepatite analyte in the sample. Within 3 minutes, the sample transferred the silver enhancing agent from the membrane strip to the reaction zone, producing a strong black line indicating the presence of the analyte.
Example 4
Based on the preferred embodiment shown in FIG. 13, the device was constructed as follows. A nitrocellulose membrane (Advanced Micro Devices, New Delhi, India) having a pore size of 8 μm and supported by a hard plastic backing plate was cut into 5 mm width and 25 mm length. The top paper wick was applied with 2 mm overlap on the membrane. Strips were formed using a Bioprinter with a 1 mg / ml solution of a single clonal anti-alpha HCG (Sigma Chemicals Ltd, UK) in water at an intensity of 1 μl / cm and 4 cm from the bottom. The strip was dried at 37 ° C. for 15 minutes. The membrane strip was then blocked by immersion for 1 minute in a mixed solution consisting of 0.1% Tween 20 and 1% polyvinylpyrrolidine (Sigma Chemicals Ltd, UK). The strip was then dried at 37 ° C. for 30 minutes. Monoclonal anti-beta HCG with 1 nm gold particles (British Biocell, UK) attached was diluted to an antibody concentration of 1 μg / ml in a solvent consisting of 0.1% Tween20 and 1% polyvinylpyrrolidine. 5 μl was weighed and applied onto individual strips of 5 × 30 mm glass fiber, approximately 2 cm from the lower end. Intensifiers and initiators from the silver enhancement kit (SELK15, British Biocell International Ltd, UK) are also applied onto individual strips made of glass fiber (Whatman, UK), each in a separate area 5 mm from the surface. It was applied by weighing 5 μl. Then, it was dried at 37 ° C. for 15 minutes. The glass fiber strip was then held in place through a double-sided adhesive tape layer on a plastic backing plate with a nitrocellulose membrane so that the strip overlapped the membrane by 1 mm. The assembled strip was placed so that the lower end was located in a microwell containing 100 μl urine from a 4 week pregnant woman. The sample caused migration of the gold complex from the glass fiber strip towards the reaction zone and reacted with the beta HCG analyte in the sample. Within 3 minutes, the sample moved silver-enhancing drug from the glass fiber strip onto the nitrocellulose membrane and further upwards into the reaction zone, creating a strong black line indicating the presence of the analyte.
Example 5
The device shown in FIG. 7 was made using a 25 mm wide and 80 mm long nitrocellulose strip (Advanced Micro Devices, India). The strips were printed with a non-dissolving ink border using a marker pen as shown by the dashed lines in FIG. This configuration does not form a separate channel for the drug. However, it allows the drug to converge towards the detection zone. The strip is about 4 cm from the bottom, using a Bioprinter, a 1 mg / ml solution of a single clone anti-alpha HCG (Sigma Chemicals Ltd, UK) in water at a concentration of 1 μl / cm across the width of the channel. Printed in the detection zone. The strip was dried at 37 ° C. for 15 minutes. The membrane strip was then blocked by immersion for 1 minute in a mixed solution consisting of 0.1% Tween 20 and 1% polyvinylpyrrolidine (Sigma Chemicals Ltd, UK). The strip was then dried at 37 ° C. for 30 minutes. Monoclonal anti-beta HCG with 1 nm gold particles (British Biocell, UK) attached was diluted to an antibody concentration of 1 μg / ml in a solvent consisting of 0.1% Tween20 and 1% polyvinylpyrrolidine. 5 μl was weighed and applied onto the strip in region 48 in FIG. 7, just on the center line, about 1 cm from the bottom edge. Both enhancer and initiator from the silver enhancement kit (SELK15, British Biocell International Ltd, UK) were applied by weighing 3 μl each to the zone indicated at 49. The two drugs are separated by about 5 mm to the left of the center line. Then, it was dried at 37 ° C. for 15 minutes. The silver enhancement agent was placed about 2 cm from the lower end, to the left of the center line. The strip was placed with the lower end located in a microwell containing 100 μl of urine from a 2 week pregnant woman. The sample caused migration of the gold complex from the strip toward the reaction zone and reacted with the beta HCG analyte in the sample. Within 3 minutes, the sample moved silver-enhancing drug from the glass fiber strip onto the nitrocellulose membrane and further upwards into the reaction zone, creating a strong black line indicating the presence of the analyte. Further sample flow from the bottom edge washed away the remaining drug from the membrane into the upper zone.
The device can perform with high sensitivity the analysis that should be done quickly in a one-step procedure. Depending on the analysis being performed, the available drugs, and the type of analysis device desired, many other configurations are possible and these form part of the present invention.

Claims (27)

An analytical device for detecting the presence of an analyte in a sample and generating a visible signal at a detection site on a support to inform the presence or absence of the analyte,
A strip device having a single channel;
The signal is generated or enhanced by a signal enhancement reaction between the labeled first binding agent and the label developing means;
The first binding agent and the label developing means are configured to be transported to the detection site by a single analysis step by application of the sample. In this case, the first binding agent and the label developing means are The analysis device, wherein the first binding agent is transported to the detection site in an order that arrives before the label developing means. (A) a porous member;
(B) the first binding agent and specifically binding to the analyte , and the porous member based on the influence of the liquid in the detection zone by a single step only by applying the sample. Said first binding agent , wherein said first binding agent comprises a label that is movable through and is not visible;
(C) either specifically binds to the analyte complementary to the binding of the first binding agent, or is competitive with the analyte for binding to the first binding agent. And a second binding agent immobilized within the detection site;
(D) It is the label developing means and can be moved into the detection site after the first binding agent under the influence of the liquid , and the invisible label is visible. Said label developing means capable of:
Analysis device according to claim 1, characterized in that it comprises a. The invisible label is a fine metal label,
3. The analytical device according to claim 2, wherein the label developing unit includes a drug that forms a solid material on the surface of the metal. 4. The analytical device according to claim 3, wherein the size of the particles of the label is 1 to 100 nm, preferably smaller than 5 nm. The analysis device according to claim 3, wherein the label is a fine-grained gold label. The analysis device according to claim 5, wherein the label developing unit includes a silver-containing drug. The label developing means is applied to the porous member such that the release of the label developing means from the porous member in the presence of the liquid is delayed from the release of the first labeled binding agent. The analysis device according to claim 2, wherein the analysis device is provided. 8. The analytical device according to claim 7, wherein the label developing means is applied in the form of a composition containing a sustained-release drug. 9. The analytical device according to claim 7, wherein the label developing means is contained in a second porous member that is in contact with the porous member. The analysis device according to claim 9, wherein the second porous member is a glass fiber pad. 11. The analysis device according to claim 7, wherein the first binding agent is applied in a composition containing a sustained-release agent. The analysis device according to any one of claims 2 to 6, wherein the release of the movable drug from the porous member film is controlled by changing the water repellency of the porous member. 7. The analytical device according to claim 2, wherein at least movement of the label developing means through the porous member is prohibited by a semipermeable barrier. The label developing means, first, the label and the label so that the film formation of the material on the label existing on the porous member forms a barrier that deflects the liquid flow toward the detection zone. The analysis device according to claim 3, wherein the analysis device is configured to abut. 15. The analysis device according to claim 1, further comprising an open housing so that the sample can be administered and the detection zone can be observed. 16. An analytical device according to any preceding claim, comprising at least one wick or wick region configured to assist in fluid flow through the device. 17. The analysis device according to claim 1, wherein a diffusion means is provided to uniformly disperse the drug prior to the reaction in the detection zone. 18. The analysis device according to claim 1, wherein the detection zone is configured to wash the detection zone between reaction stages. 19. The analytical device according to claim 18, wherein a liquid sample that may contain an analytical substance is used as a cleaning liquid. 20. The analytical device according to claim 19, wherein filter means are provided for removing unwanted elements from the cleaning liquid. Configured for use in serum analysis,
21. The analytical device according to claim 20, wherein the filter means comprises an anti-antibody capable of removing the antibody from the serum sample. The labeled first binding agent comprises a labeled nucleic acid probe;
The analysis device according to any one of claims 1 to 21, wherein the analysis substance includes a nucleic acid string fixed in the detection zone. A method for detecting the presence of an analyte in a liquid sample,
Applying the liquid sample to the analytical device according to any of claims 1 to 22,
A method comprising recording whether a visible signal is generated. Used for diagnostic analysis ,
In order to create a signal that indicates the presence or absence of the analyte, the liquid can be moved through the porous member,
Comprising a first agent and a second agent configured to react with each other during the analysis so as to form a physical barrier that deflects liquid flow through the porous member. The analysis device according to any one of claims 1 to 21. Multiple reaction steps are provided at the detection site on the porous member,
During at least two of the reactions, a cleaning liquid is applied to the site;
The analysis device according to any one of claims 1 to 21, wherein the cleaning liquid includes a part of the sample that has already passed through the filter means provided on the member. Used for serum analysis,
The filter means comprises an anti-antibody band immobilized on the surface of the porous member;
26. The band is fixed at a position where a part of a sample intended to be used as a washing liquid passes through the band before reaching a detection site. The described analytical device. 27. A kit comprising a porous member configured for use in the analytical device of claim 26.

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